Background
Cervical cancer, which accounts for the second most common malignancy among women worldwide, is highly radio-resistant, often resulting in local treatment failure [
1]. For locally advanced disease, radiation is combined with low-dose chemotherapy; however, this modality often leads to severe toxicity. Complementary and Alternative Medicine (CAM) is recently becoming a popular treatment for various cancers among which herbal medicine is one of the methods used in cancer therapy [
2,
3]. Currently, plants, vegetables, herbs and spices used in folk and traditional medicine have been accepted as one of the main sources of chemopreventive drugs [
4‐
8]. Traditional medicine that includes herbal medicine has been used from time immemorial to treat chronic ailments such as cancer. Recently, scientific studies support herbal medicine as potent anti-cancer drug candidates [
9‐
13].
Cinnamon, a widely used food spice, has been shown to exhibit diverse biological functions including anti-inflammatory [
14], anti-oxidant [
15,
16], anti-microbial [
15,
17], and anti-diabetic effects [
18‐
20]. Recently, the anti-tumor activity of cinnamon has been shown both in vitro [
21‐
23] and
in vivo [
10]. Cinnamaldehyde, the bioactive component of cinnamon, has been shown to inhibit proliferation of several human cancer cell lines including breast, leukemia, ovarian, and lung tumor cells [
24]. Recently, we reported a comparative analysis of cytotoxic effect of aqueous extract of cinnamon (ACE) from
C. zeylanicum with that of commercial cinnamaldehyde on a variety of cell lines [
23]. Compared to the commercial cinnamaldehyde, ACE proved to be more cytotoxic owing to the presence of polyphenolic compounds, besides cinnamaldehyde, that may act synergistically to induce enhanced cytotoxicity.
In the present work, we have reported the putative mechanism of cancer cell growth inhibition by aqueous cinnamon extract (ACE-c), from the bark of Cinnamomum cassia L. family Lauraceae, in a human cervical cancer cell line, SiHa. We observed that cinnamon altered the growth kinetics of cells in a dose-dependent manner. Our colony formation and soft agar assays demonstrated that the number of colonies in cells treated with ACE-c was less compared to the untreated control cells. The ACE-c treated cells exhibited slow migration potential compared to the control cells that could be explained due to reduced MMP-2 expression in the former. Cinnamon extract increased the intracellular calcium that might be responsible for the loss of mitochondrial membrane potential (Δψm), finally leading to cellular apoptosis.
Methods
Reagents
Tissue culture plasticware was purchased from BD Biosciences, CA, USA; Axygen Scientific Inc, CA, USA and Nunc, Roskilde, Denmark. Dulbecco's Modified Eagles Medium (DMEM) was obtained from Himedia Corporation, Mumbai, India. Penicillin and streptomycin were obtained from Gibco BRL, CA, USA. Fetal bovine serum was purchased from Moregate Biotech, Australia, N. Z and 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenylthiazolium bromide (MTT), FCCP, JC-1 and TMRE were purchased from Sigma-Aldrich (St. Louis, MO). Her-2 antibody was purchased from Santa Cruz Biotechnology, CA, USA, Donkey anti-Mouse IgG Cy-3conjugate (Millipore, MA) and Annexin V-FITC apoptosis kit #3 from Invitrogen (CA, USA). All other common reagents were procured from Qualigens fine chemicals (Mumbai, India).
ACE-c preparation and characterization
The bark of
Cinnamomum cassia was purchased from Shivam Ayurvedics Pune, Maharashtra, India with voucher specimen number for
Cinnamomum cassia bark was 104. The sample was authenticated from Regional Research Institute (AY) Kothrud, Pune (ref no.1045). The bark was weighed, powdered and extracted in double distilled water (the ratio of cinnamon: water used was 1:16) in a hot water extractor [
25]. The resulting extract was centrifuged at 13000 rpm for 15 min to remove the particulate matter. The supernatant was further filter-sterilized using swiney filter (pore size, 0.45 μm) and the resultant filtrate was stored in aliquots at -80°C until use. The bark identity was further confirmed by detecting the marker molecule cinnamaldehyde in ACE-
c by HPTLC analysis as described previously [
23,
26]. The total polyphenol content of ACE-c was measured by Folin-Ciocalteau method as described previously [
23,
26].
Cell culture
The human cervical carcinoma cell line, SiHa, used in the study was obtained from National Centre for Cell Science (NCCS), Pune, India. The cells were grown in DMEM containing 2 mM L-glutamine supplemented with 10% fetal bovine serum and 100 U/ml of penicillin-streptomycin. The cells were incubated in a humidified 5% CO2 incubator at 37°C.
Cell viability
The cell viability was determined by MTT dye uptake as described previously [
23]. Briefly, SiHa cells were seeded at a density of 1 × 10
5 cells/ml density in 96-well plates. An untreated group was kept as a negative control. The aqueous cinnamon extract (ACE-
c) was added at following concentrations: 10, 20, 40, 80, 160 and 320 μg/ml, in wells in triplicates. The MTT solution (5 mg/ml) was added to each well, and the cells were cultured for another 4 h at 37°C in 5% CO
2 incubator. The formazan crystals formed were dissolved by addition of 90 μl of SDS-DMF (20% SDS in 50% DMF). After 15 min, the amount of colored formazan derivative was determined by measuring optical density (OD) using the ELISA microplate reader (Biorad, Hercules, CA) at 570 nm (OD
570-630 nm). The percentage viability was calculated as: % Viability = [OD of treated cells/OD of control cells] × 100
Cell growth analysis
SiHa cells were seeded at a density of 1 × 105 cells/ml in 24-well plates in triplicates. Next day, the cells were dosed with different concentrations of ACE-c (0, 10, 20, 40 and 80 μg/ml) and grown for 24, 48 and 72 h. The cells were harvested and counted for viability using trypan blue dye exclusion method.
The cells were plated at a seeding density of 1 × 10
3 cells/ml in 6-well plates. After 24 h, the cells were exposed to various concentrations of ACE-
c: 0, 10, 20, 40, and 80 μg/ml. Plates were incubated at 37°C in a 5% CO
2 incubator for one week. This was followed by fixing the colonies with 4% paraformaldehyde and staining with 0.5% crystal violet [
27]. The colonies were photographed with Sony DSC-S75 cyber-shot camera.
Soft agar assay
Control SiHa cells (5 × 10
3 cells/ml) as well as cells treated with different concentrations of ACE-
c (10-80 μg/ml) were mixed at 40°C with 0.35% agarose (DNA grade, GIBCO BRL, CA, USA) in culture medium and gelled at room temperature for 20 min over a previously gelled layer of 0.5% agarose in culture medium in 6-well plates. After incubation for 10 days, colonies were photographed directly using an Axiovert 200 M microscope (Carl Zeiss, Germany) and counted [
27].
Wound healing assay
Cells were plated at a seeding density of 4 × 105 cells/ml in 24-well plates and grown overnight at 37°C in 5% CO2 incubator. An artificial wound was made with 10 μl micropipette after 6 h serum starvation in control cells as well as cells treated with different concentrations of ACE-c (10-80 μg/ml). Time-lapse imaging of migrating cells was performed on Nikon Eclipse TE2000-E microscope (Nikon, Tokyo, Japan) over 15 h in serum containing medium in a humidified chamber at 37°C and 5% CO2 atmosphere. Images were obtained every 20 min using a 10× phase objective of NA 0.25 and analyzed by image analysis software Metamorph Universal Imaging, USA. The average migration rate in μm/h was calculated and graphs were plotted using Microsoft Excel and Sigma plot program.
RT-PCR analysis
The total cellular RNA from control as well as cells treated with different doses of ACE-c (0-80 μg/ml) was extracted by a one-step acid guanidine isothiocyanate-phenol method using TRI reagent (Sigma, St. Louis, MO). RNA was precipitated with isopropanol and the concentration was estimated by spectrophotometer (Biorad, SmartSpec™ 3000). Ten microgram of total RNA was used for each RT-PCR reaction. Fifty units of Moloney murine leukemia virus reverse transcriptase (MMuLV) (Bangalore Genei, Banglore, India) were added in a typical 50 μl reaction (10 μg RNA, 1× first-strand buffer, 1 mM DTT, 2.5 mM dNTPs, 50 ng/μl random primers and 15 U/μl RNAse i) and incubated for 1 h at 42°C followed by incubation at 95°C for 5 min. The purified cDNA template was amplified using different sets of primers. The primers used were as follows: β-actin-F: 5'-taccactggcatcgtgatggact-3'; β-actin-R: 5'-tttctgcatcctgtcggaaat-3'; MMP-2-F: 5'-ggctggtcagtggcttggggta-3'; MMP-2-R: 5'-agatcttcttcttcaaggaccggtt-3'. PCRs were performed in 25 μl volume in which 1× PCR buffer, 2.5 mM dNTPs, 1.5 mM MgCl2, 1 U of Taq polymerase and 100 ng of the specific primers were added. A brief initial denaturation at 95°C for 5 min was followed by 35 cycles with the following steps: 95°C for 1 min, annealing at 55-55.2°C for 1 min and extension at 72°C for 1 min. RT-PCR products were then separated on a 1.2% agarose gel and visualized by staining with ethidium bromide. The intensities of the bands corresponding to the RT-PCR products were quantified using phosphorimager (Alpha Imager using Alpha Ease FC software, Alpha Innotech) and normalized with respect to the β-actin product.
Gelatin zymography
The Gelatin zymography was performed to detect the presence of extracellular MMP-2 [
28]. The conditioned medium of control cells as well as cells treated with 80 μg/ml ACE-
c was collected and concentrated in Centricon YM-30 tubes (Millipore, MA). Both the control as well as the treated samples containing equal amount of total proteins were mixed with sample buffer (2% SDS, 25% glycerol, 0.1% bromophenol blue and 60 mM Tris- HCl pH 6.8) and loaded onto 7.5% SDS-polyacrylamide gel containing gelatin (0.5 mg/ml). The gel was washed with 0.25% Triton X-100 and incubated overnight in incubation buffer (150 mM NaCl, 100 mM CaCl
2, 50 mM Tris-HCl pH 7.5, 1% Triton X- 100, 0.02% NaN
3) at 37°C. The gel was stained with staining solution (0.1% Coomassie Brilliant blue R-250 in 40% isopropanol) and destained in 7% acetic acid. Gelatinolytic activity was detected as unstained bands on a blue background. The quantitation of bands in control and treated samples was performed by densitometric analysis on Alpha Imager using Alpha Ease FC software, Alpha Innotech.
Immunoblotting
Cell extracts were prepared from control as well as cells treated with different concentrations of ACE-c: (0-80 μg/ml). Briefly, the cell pellet was resuspended in 80 μl lysis buffer containing 50 mM Tris (pH 7.4), 5 mM EDTA, 0.5% NP40, 50 mM NaF, 1 mM DTT, 0.1 mM PMSF, 0.5 μg/ml leupeptin (Pro-pure Amersco, Solon, USA), 1 μg/ml pepstatin (Amresco, Solon, USA), 150 mM NaCl, 0.5 μg/ml aprotinin (Amersco, Solon, USA) and protease inhibitor cocktail (Roche, Lewes, UK) and incubated on ice for 1 h with intermittent mixing. The extract was centrifuged for 20 min at 4°C at 12000 rpm. The protein was estimated using Bradford reagent (Biorad Laboratories Inc, CA, USA). Equal amount of protein was loaded on a 10% SDS-polyacrylamide gel and transferred electrophoretically to Amersham Hybond-P PVDF membrane (GE Healthcare, UK) in sodium phosphate buffer (pH 6.8). The membrane was blocked in 5% BSA in TST and incubated at room temperature for 1 h with mouse monoclonal antibody for Her-2 and tubulin (Santacruz, CA, USA) at a 1:1000 and 1:2500 dilution, respectively. The membrane was washed in TST and incubated with donkey anti mouse IgG HRP conjugate at 1:5000 (for Her-2) and 1:3000 (for tubulin) dilutions. Proteins were visualized using a chemiluminescence kit (Amersham ECL Advance western blotting detection kit, GE Healthcare, UK) and densitometric analysis of X-ray films was performed on Alpha Imager using Alpha Ease FC software, Alpha Innotech.
Measurement of Apoptosis
The cells were plated at a seeding density of 5 × 105 cells/well and treated with different concentrations of ACE-c: (0-80 μg/ml). After 24 h of treatment, the cells were harvested and washed with PBS twice. Cells were stained with Annexin V-FITC following the manufacturer's instructions (Annexin V-FITC apoptosis kit #3, Invitrogen) and analyzed for apoptosis by FACS using CellQuest Software.
Intracellular calcium measurement by flow cytometry
Intracellular Ca
2+ levels were analyzed in control cells as well as cells treated with different doses of ACE-
c: (0-80 μg/ml) by flow cytometry [
29]. Cells were loaded with 5 μM Fluo-3/AM (Sigma, St. Louis, MO) and 100 μg/ml of Pluronic F127 (Sigma, St. Louis, MO) in centrifuge tubes and incubated at 37°C, 5% CO
2 for 1 h in the dark. The cells were resuspended after every 20 min to ensure even dye loading. The cell pellets were washed twice with 0.9% saline and finally resuspended in 3 ml Hank's Balanced Salt Solution (HBSS) in FACS tubes. Ionomycin (30 μM) was used as a positive control. Fluorescence intensities were measured at 525 nm by FACS Calibur (Becton Dickinson Immunocytometry Systems, San Jose, CA) to obtain baseline readings. Mean channel fluorescence intensities were calculated using CellQuest software.
Detection of Mitochondrial Membrane Potential (Δψm) using JC-1
Mitochondrial membrane potential was estimated using 2.5 μg/ml JC-1 fluorescent dye either by confocal microscopy or by flow cytometry. For confocal studies, cells were seeded at a density of 1 × 10
5 cells/ml on coverslips in 6-well plates. After 24 h, cells were treated with different concentrations of ACE-
c: (0-80 μg/ml). Next day, the media was removed and the cells were incubated with fresh culture medium containing JC-1 dye for 30 min at 37°C in the dark. Cells on coverslips were washed with PBS twice and fixed with 2.5% paraformaldehyde made in 200 mM HEPES buffer for 15 min at room temperature followed by PBS wash. The coveslips were mounted in antifade mounting medium containing DAPI (Ultracruz mounting medium, Santacruz) on glass slides. The cells were then analyzed for JC-1 uptake by using Zeiss LSM510 META confocal laser scanning microscope (Zeiss, Thornwood, NY) having LSM Image Examine software. For
Δψm detection by flow cytometry [
30], 5 × 10
5 cells were plated in 6-well plates. The cells were treated with different concentrations of ACE-
c (0-80 μg/ml). Twenty four hours post treatment; the cells were harvested, washed with PBS and incubated with culture medium containing JC-1 for 30 min at 37°C in the dark. Cells were washed in PBS twice and analyzed for
Δψm using FACS. FCCP (10 μM) was used as a positive control. The fluorescence intensities were measured at 527 nm (green) and 590 nm (red). Analysis was done by CellQuest software.
Immunofluorescence microscopy
For immunostaining SiHa cells were plated on coverslips in 6-well plates at a seeding density of 2 × 105 cells/ml. After 24 h, the cells were dosed with different concentrations of ACE-c (0-80 μg/ml). Twenty four hours post-treatment; the cells were washed with PBS and fixed in 2.5% paraformaldehyde made in 200 mM HEPES buffer for 15 min at room temperature. Cells were washed for 5 min in PBS, permeabilized with 0.1% Triton X-100 in PBS for 5 min and blocked in 10% FBS (made in PBS) for 1 h. For detection, the cells were incubated with Her-2 antibody (Santa Cruz Biotechnology, Santa Cruz, CA) that was diluted in blocking buffer at 1:100 dilution. After washing with PBS, the cells were incubated with the secondary antibody [CY3-conjugated antimouse immunoglobulin (Millipore)] at a dilution of 1:300. Slides were then mounted in antifade mounting medium (Ultracruz mounting medium, Santacruz) and analyzed with a Zeiss LSM 510 META confocal laser scanning microscope (Zeiss, Thornwood, NY) using LSM Image Examine software.
Statistical analysis
All experiments were performed in triplicates and repeated at least five times and the data were presented as mean ± SD. Statistical analysis was conducted with the SigmaStat 3.5 program (Systat Software, Inc.) using one-way ANOVA. The α level used for comparisons was α = 0.05.
Discussion
Dietary constituents may display promising chemopreventive and chemotherapeutic potential and thus ameliorate the side effects associated with conventional chemotherapy. Recently, more attention is being focused on complementary and alternative medicine (CAM) as an alternative therapeutic modality for treatment of cancer patients [
2,
3,
9‐
13,
40].
In the present study, we have reported the anti-cancer potential of cinnamon extract in vitro in a human cervical cancer cell line and have elucidated the possible underlying mechanism. The anti-tumor activity of cinnamon has been reported
in vitro [
21‐
23] as well as in
vivo [
10]; however, its role in cervical cancer remained to be elucidated. We found that the aqueous cinnamon extract significantly affected the growth rate of SiHa cells in a dose-dependent manner. This data was further supported by results from colony formation and soft agar assays, which demonstrated statistically significant reduction in the number of colonies in ACE-
c treated cells compared to the untreated control cells. Thus, cinnamon could be proposed to be a promising candidate for restricting the growth of cervical cancer cells.
It is well known that metastasis, being one of the major causes of mortality in cancer, involves various steps such as cancer cell adhesion, invasion, and migration [
41]. Thus, to examine the effect of cinnamon extract on migration of SiHa cells, wound healing assays were performed on untreated control and ACE-
c treated cells. Interestingly, cinnamon reduced the migration of cancer cells in a significant manner, further strengthening its potential use as an anti-cancer drug in cervical cancer.
One of the key steps in the invasive progress of cancer cells is the degradation of extracellular matrix (ECM) proteins by a family of zinc-binding enzymes called as matrix metalloproteinases [
42]. To elucidate the reason behind the poor migration of ACE-
c treated cells, we tested the expression of MMP-2 (gelatinase) in control as well as cinnamon-treated cells. A significant decrease in the expression of MMP-2 was observed both at mRNA as well as protein levels in ACE-
c treated cells that could be the reason for their reduced migration capability compared to the control cells. Thus, downregulation of MMP-2 expression by cinnamon could be regarded as a rational approach towards metastatic disease therapy in cervical cancer.
It is well-known that Her-2/Erb2, a transmembrane receptor protein with tyrosine kinase activity from EGF3-receptor family, is a critical marker of cervical and breast cancer. Moreover, it has been shown that Her2 overexpression is related with the invasion capacity of the tumor cells that is related partly with the up-regulation of MMP-2 and MMP-9 expression as well as proteolytic activity [
32,
33]. Interestingly, we found that cinnamon could effectively and significantly down-regulate the expression of Her-2 in SiHa cells. Thus, downregulation of Her-2 oncoprotein expression by cinnamon could be correlated with the reduction in the expression of MMP-2 protein. These leads could be explored in detail to further establish the antineoplastic activity of cinnamon in cervical cancer that would in turn emphasize the chemopreventive potential of natural products.
Apoptosis plays a key role in the regulation of normal tissue homeostasis and participates in the elimination of abnormal cells. Most of the antitumor drugs kill the cancer cells by stimulating the apoptotic pathway [
43]. To test whether cinnamon could induce apoptosis in cervical cancer cell line SiHa, we carried out apoptosis studies. At an effective ACE-
c concentration of 80 μg/ml, a significant proportion of cells were observed to undergo apoptosis compared to the control cells. To further elucidate the mechanism of apoptosis, we tested whether cinnamon could modulate calcium flux as the latter is known to be one of the major mediators of apoptosis.
Intracellular Ca
2+ trafficking is known to govern a number of vital cellular functions that affect cell survival. Cytosolic calcium, (Ca
2+)
c, is usually maintained at lower level (~100 nmol/L) compared to the extracellular concentration (~1 mmol/L). The cells regulate (Ca
2+)
c primarily by regulating the Ca
2+ trafficking across the plasma membrane and in and out of key organelles, such as the endoplasmic reticulum and the mitochondria [
42]. The endoplasmic reticulum is the largest reservoir of Ca
2+ in normal cells whereas mitochondrial levels of Ca
2+ are quite low. But during apoptosis, mitochondria are known to accumulate Ca
2+, especially when the (Ca
2+)
c level is high [
35,
37‐
39]. Increase in mitochondrial calcium, (Ca
2+)
m, induces apoptosis resulting into loss of Δψ
m, expansion of the matrix, and the rupture of the outer mitochondrial membrane [
36]. Interestingly, at 80 μg/ml concentration of cinnamon extract, there was a significant increase in the levels of intracellular calcium in SiHa cells that could result into their apoptosis.
Since cinnamon increased intracellular calcium levels as well as induced apoptosis in cervical cancer cells, we wanted to know the status of mitochondrial membrane potential in these cells. Moreover, mitochondria are known to accumulate Ca
2+ during apoptosis especially when the cytosolic calcium level is high [
37‐
39,
44]. Thus, we tested the Δψ
m in cinnamon treated cells by using the fluorescent dye, JC-1 that aggregates into healthy mitochondria and fluoresces red. Upon mitochondrial collapse in apoptotic cells, JC-1 dye no longer accumulates and instead is distributed throughout the cell resulting into decrease in red fluorescence. In accordance with this, we found that ACE-
c indeed disrupted the mitochondrial membrane potential as observed by decrease in the intensity of red fluorescence. FCCP, a drug known to disrupt the transmembrane potential of mitochondria [
45], was used as a positive control. Thus, the increased intracellular calcium induced by ACE-c might be associated with the observed decline in mitochondrial membrane potential.
Dietary polyphenols have recently invited a great deal of attention owing to their chemopreventive properties [
46‐
48]. They can modulate the process of carcinogenesis through several mechanisms. Interestingly, polyphenols seem to play dual roles (either protective or therapeutic) under different situations. For example, cinnamon polyphenols have been recently shown to play a protective role by attenuating the decline in mitochondrial membrane potential induced by ischemic injury in C6 glioma cells [
49]. On the other hand, in our case, we observe that cinnamon extract, which contains a mixture of polyphenols together with cinnamaldehyde as the major bioactive component, plays a therapeutic role in cervical cancer cells through depolarization of the mitochondrial membrane potential resulting into cellular apoptosis. These natural products seem to work in a tightly regulated manner wherein they switch their roles either towards protective or therapeutic side depending upon either the amount of the drug being used or upon the cellular phenotype [
50]. For example, resveratrol, another polyphenol, has also been shown to play a dual role, either protective [
51‐
53] or therapeutic [
54]. Based on all these observations, our data strongly implicates that cinnamon could be proposed to be a potent antineoplastic agent in cervical cancer wherein it could induce apoptosis through increase in calcium flux as well as through loss of mitochondrial membrane potential.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
RKG designed the study and drafted the manuscript. SJK and ASC have carried out all the experiments. SK had participated in cell growth analysis and RT-PCR experiments. SAS contributed to the FACS analysis. SC has helped in time-lapse study. All the authors read and approved the final version of the manuscript.